TY - JOUR
T1 - Identification of a DNA supercoiling activity in Saccharomyces cerevisiae
AU - Koo, Hyeon sook
AU - Lau, Kawai
AU - Wu, Hai young
AU - Liu, Leroy F.
N1 - Funding Information:
We thank Drs. John Nitiss, James Wang and Rolf Sternglanz for providing us with yeast strains. This work was supported by NIH grant GM27731. LFL is a recipient of the George Hitchings Award from the Burroughs Wellcome Fund.
PY - 1992/10/11
Y1 - 1992/10/11
N2 - A sensitive and simple method for the quantitatlon of human DNA is described. This method Is based on probe hybridization to a human alpha satellite locus, D17Z1. The biotlnylated probe is hybridized to sample DNA immobilized on nylon membrane. The subsequent binding of streptavldln-horseradish peroxidase to the bound probe allows for chemlluminescent detection using a luminol-based reagent and X-ray film. Less than 150 pg of human DNA can easily be detected with a 15 minute exposure. The entire procedure can be performed in 1.5 hours. Microgram quantities of non-human DNA have been tested and the results indicate very high specificity for human DNA. The data on film can be scanned into a computer and a commercially available program can be used to create a standard curve where DNA quantity is plotted against the mean density of each slot blot signal. The methods described can also be applied to the very sensitive determination of quantity and quality (size) of DNA on Southern blots. The high sensitivity of this quantltation method requires the consumption of only a fraction of sample for analysis. Determination of DNA quantity is necessary for RFLP and many PCR-based tests where optimal results are obtained only with a relatively narrow range of DNA quantities. The specificity of this quantitation method for human DNA will be useful for the analysis of samples that may also contain bacterial or other non-human DNA, for example forensic evidence samples, ancient DNA samples, or clinical samples.
AB - A sensitive and simple method for the quantitatlon of human DNA is described. This method Is based on probe hybridization to a human alpha satellite locus, D17Z1. The biotlnylated probe is hybridized to sample DNA immobilized on nylon membrane. The subsequent binding of streptavldln-horseradish peroxidase to the bound probe allows for chemlluminescent detection using a luminol-based reagent and X-ray film. Less than 150 pg of human DNA can easily be detected with a 15 minute exposure. The entire procedure can be performed in 1.5 hours. Microgram quantities of non-human DNA have been tested and the results indicate very high specificity for human DNA. The data on film can be scanned into a computer and a commercially available program can be used to create a standard curve where DNA quantity is plotted against the mean density of each slot blot signal. The methods described can also be applied to the very sensitive determination of quantity and quality (size) of DNA on Southern blots. The high sensitivity of this quantltation method requires the consumption of only a fraction of sample for analysis. Determination of DNA quantity is necessary for RFLP and many PCR-based tests where optimal results are obtained only with a relatively narrow range of DNA quantities. The specificity of this quantitation method for human DNA will be useful for the analysis of samples that may also contain bacterial or other non-human DNA, for example forensic evidence samples, ancient DNA samples, or clinical samples.
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U2 - 10.1093/nar/20.19.5067
DO - 10.1093/nar/20.19.5067
M3 - Article
C2 - 1329038
AN - SCOPUS:0026712371
SN - 0305-1048
VL - 20
SP - 5067
EP - 5072
JO - Nucleic Acids Research
JF - Nucleic Acids Research
IS - 19
ER -